Mercurial > repos > weilong-guo > bs_seeker2

comparison BSseeker2/bs_align/output.py @ 0:e6df770c0e58 draft

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Initial upload
author weilong-guo
date Fri, 12 Jul 2013 18:47:28 -0400
parents
children 8b26adf64adc
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-1:000000000000 0:e6df770c0e58
1 try :
2 import pysam
3 except ImportError :
4 print "[Error] It seems that you haven't install \"pysam\" package.. Please do it before you run this script."
5 exit(-1)
6
7 import sys
8 from bs_align_utils import *
9
10 BAM = 'bam'
11 SAM = 'sam'
12 BS_SEEKER1 = 'bs_seeker1'
13
14 formats = [BAM, SAM, BS_SEEKER1]
15
16 class outfile:
17 def __init__(self, filename, format, chrom_len, cmd_line, suppress_SAM_header):
18 self.filename = filename
19 self.format = format
20 self.chrom_ids = dict((k, i) for i, k in enumerate(sorted(chrom_len)))
21
22 if format == BS_SEEKER1:
23 self.f = open(filename, 'w')
24 elif format in [SAM, BAM]:
25 header = { 'HD' : { 'VN': '1.0'},
26 'SQ' : [ {'LN' : chrom_len[c], 'SN' : c} for c in sorted(chrom_len) ],
27 'PG' : [ { 'ID' : 1, 'PN' : 'BS Seeker 2', 'CL' : cmd_line} ]
28 }
29 self.f = pysam.Samfile(filename, 'w' + ('b' if format == BAM else ('' if suppress_SAM_header else 'h')), header = header)
30
31
32
33 def close(self):
34 self.f.close()
35
36 def store(self, qname, N_mismatch, FR, refname, strand, pos, cigar, original_BS, methy, STEVE, rnext = -1, pnext = -1, qual = None, output_genome = None,
37 rrbs = False, my_region_serial = -1, my_region_start = 0, my_region_end = 0):
38
39 if self.format == BS_SEEKER1:
40
41 # remove the soft clipped bases from the read
42 # this is done for backwards compatibility with the old format
43 r_start, r_end, _ = get_read_start_end_and_genome_length(cigar)
44 original_BS = original_BS[r_start : r_end]
45
46 if rrbs:
47 self.f.write('%s\t%2d\t%s\t%s%s%s\t%s\t%s\t%s\t%d\n' % (qname, N_mismatch, FR, refname, strand, str(pos+1).zfill(10), output_genome, original_BS, methy, STEVE))
48 else:
49 self.f.write('%s\t%2d\t%s\t%s%s%s\t%s\t%s\t%s\t%d\t%d\t%d\t%d\n' % (qname, N_mismatch, FR, refname, strand, str(pos+1).zfill(10), output_genome, original_BS, methy, my_region_serial, my_region_start, my_region_end, STEVE))
50
51
52 elif self.format == BAM or self.format == SAM:
53
54 a = pysam.AlignedRead()
55 a.qname = qname
56 a.seq = original_BS if strand == '+' else reverse_compl_seq(original_BS)
57 a.flag = 0x10 if strand == '-' else 0
58 a.tid = self.chrom_ids[refname]
59 a.pos = pos
60 a.mapq = 255
61 a.cigar = cigar if strand == '+' else list(reversed(cigar))
62 a.rnext = rnext if rnext == -1 else self.chrom_ids[rnext]
63 a.pnext = pnext
64 a.qual= qual
65 if rrbs:
66 a.tags = (('XO', FR),
67 ('XS', STEVE),
68 ('NM', N_mismatch),
69 ('XM', methy),
70 ('XG', output_genome),
71 ('YR', my_region_serial),
72 ('YS', my_region_start),
73 ('YE', my_region_end)
74 )
75
76 else:
77 a.tags = (('XO', FR),
78 ('XS', STEVE),
79 ('NM', N_mismatch),
80 ('XM', methy),
81 ('XG', output_genome))
82
83 self.f.write(a)